Phage Lytic Protein CHAPSH3b Encapsulated in Niosomes and Gelatine Films-Reference-Cited by-同舟云学术

Phage Lytic Protein CHAPSH3b Encapsulated in Niosomes and Gelatine Films

Published:2024-01-06 Issue:1 Volume:12 Page:119
ISSN:2076-2607
Container-title:Microorganisms
language:en
Short-container-title:Microorganisms

Author:

Marchianò Verdiana¹²^ORCID,Duarte Ana Catarina³⁴^ORCID,Agún Seila³⁴,Luque Susana²^ORCID,Marcet Ismael²^ORCID,Fernández Lucía³⁴^ORCID,Matos María²⁵^ORCID,Blanco Mª del Carmen¹⁵^ORCID,García Pilar³⁴^ORCID,Gutiérrez Gemma²⁵^ORCID

Affiliation:

1. Department of Physical and Analytical Chemistry, University of Oviedo, Julián Clavería 8, 33006 Oviedo, Spain

2. Department of Chemical and Environmental Engineering, University of Oviedo, Julián Clavería 8, 33006 Oviedo, Spain

3. Instituto de Productos Lácteos de Asturias (IPLA-CSIC), Paseo Río Linares s/n., 33300 Villaviciosa, Spain

4. DairySafe Group, Instituto de Investigación Sanitaria del Principado de Asturias (ISPA), 33011 Oviedo, Spain

5. Instituto Universitario de Biotecnología de Asturias, University of Oviedo, 33006 Oviedo, Spain

Abstract

Antimicrobial resistance (AMR) has emerged as a global health challenge, sparking worldwide interest in exploring the antimicrobial potential of natural compounds as an alternative to conventional antibiotics. In recent years, one area of focus has been the utilization of bacteriophages and their derivative proteins. Specifically, phage lytic proteins, or endolysins, are specialized enzymes that induce bacterial cell lysis and can be efficiently produced and purified following overexpression in bacteria. Nonetheless, a significant limitation of these proteins is their vulnerability to certain environmental conditions, which may impair their effectiveness. Encapsulating endolysins in vesicles could mitigate this issue by providing added protection to the proteins, enabling controlled release, and enhancing their stability, particularly at temperatures around 4 °C. In this work, the chimeric lytic protein CHAPSH3b was encapsulated within non-ionic surfactant-based vesicles (niosomes) created using the thin film hydrating method (TFH). These protein-loaded niosomes were then characterized, revealing sizes in the range of 30–80 nm, zeta potentials between 30 and 50 mV, and an encapsulation efficiency (EE) of 50–60%. Additionally, with the objective of exploring their potential application in the food industry, these endolysin-loaded niosomes were incorporated into gelatine films. This was carried out to evaluate their stability and antimicrobial efficacy against Staphylococcus aureus.

Publisher

MDPI AG

Link

https://www.mdpi.com/2076-2607/12/1/119/pdf

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